Effective inhibition of human cytomegalovirus gene expression and replication by a ribozyme derived from the catalytic RNA subunit of RNase P from
            <i>Escherichia coli</i>

Trang, Phong; Lee, Manfred; Nepomuceno, Edward; Kim, Joe; Zhu, Hua; Liu, Fenyong

doi:10.1073/pnas.100101797

Cited by 70 publications

(175 citation statements)

References 35 publications

(51 reference statements)

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“…M1 RNA may be converted to an endoribonuclease that specifically cleaves other RNAs through the covalent attachment of a guide sequence (GS) which is complementary to the target RNA and to the 39 end of the M1 RNA. Reduced levels of virus replication of herpes simplex virus (Trang et al, 2000a) and cytomegalovirus (Trang et al, 2000b) in cell culture have been reported with the use of M1GSs.…”

mentioning

confidence: 98%

Characterization of the structure and variability of an internal region of hepatitis C virus RNA for M1 RNA guide sequence ribozyme targeting

Nadal

Robertson

Guàrdia

et al. 2003

Journal of General Virology

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Accessibility to folded RNA and low potential of variation in the target RNA are crucial requirements for ribozyme therapy against virus infections. In hepatitis C virus (HCV), the sequence of the 59UTR is conserved but the highly folded RNA structure severely limits the number of accessible sites. To expand investigation of targeting in the HCV genome, we have considered an internal genomic region whose sequence variation has been widely investigated and which has a particularly conserved RNA structure, which makes it accessible to the human RNase P in vitro. We have first mapped the accessibility of the genomic RNA to complementary DNAs within this internal genomic region. We performed a kinetic and thermodynamic study. Accordingly, we have designed and assayed four RNase P M1 RNA guide sequence ribozymes targeted to the selected sites. Considerations of RNA structural accessibility and sequence variation indicate that several target sites should be defined for simultaneous attack.

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mentioning

confidence: 98%

Characterization of the structure and variability of an internal region of hepatitis C virus RNA for M1 RNA guide sequence ribozyme targeting

Nadal

Robertson

Guàrdia

et al. 2003

Journal of General Virology

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“…We constructed functional ribozyme M1-A by linking the 3′ terminus of M1 RNA with a guide sequence of 18 nucleotides that is complementary to the targeted M80.5 mRNA sequence. Control "inactive" ribozyme M1-B was constructed to contain the same guide sequence and derived from C102 RNA, an M1 mutant that contained point mutations at the active P4 domain abolishing its catalytic activity (9). To determine if M1GS ribozyme with an incorrect guide sequence could affect the level of the target mRNA, ribozyme M1-TK1, which was derived from M1 RNA and targeted the HSV-1 thymidine kinase (TK) mRNA (9), was also used in the analysis.…”

Section: Resultsmentioning

confidence: 99%

“…Control "inactive" ribozyme M1-B was constructed to contain the same guide sequence and derived from C102 RNA, an M1 mutant that contained point mutations at the active P4 domain abolishing its catalytic activity (9). To determine if M1GS ribozyme with an incorrect guide sequence could affect the level of the target mRNA, ribozyme M1-TK1, which was derived from M1 RNA and targeted the HSV-1 thymidine kinase (TK) mRNA (9), was also used in the analysis. We observed in vitro cleavage of an M80.5 mRNA substrate by M1-A, but not M1-B or M1-TK1 (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…The DNA sequence for the M80.5 mRNA substrate was constructed by annealing primers AF25 (5′-GGAATTCTAATAC-GACTCACTATAG-3′) and sm80.5 (5′-CGGGATCCGCCCGACTGAGGTAGACGC-GGTGGTTCATCCTATAGTG AGTCGTATTA-3′), followed by PCR. Mutant ribozyme C102 contains several point mutations (e.g., A 347 C 348 → C 347 U 348 , (9). The DNA sequences that encode ribozymes M1-A and M1-B were constructed by PCR using constructs pFL117 and pC102 (9), which contained the DNA sequences of the M1 and C102 ribozymes, as the templates and primers AF25 and M1m80.5 (5′-CCCGCTCGAGAAAAAATGGTGCGTCTACCTCAGTC-GGGTGTGGAATTGTG-3′) as 5′ and 3′ primers, respectively.…”

Section: Methodsmentioning

confidence: 99%

“…1 A and B) (6, 7). M1GS RNAs efficiently cleave target cellular and viral mRNAs in vitro and block their expression in cultured cells (8,9). The M1GS-based strategy represents a distinctive nucleic-acid-based interference approach because of the use of M1 RNA, an efficient naturally occurring RNA catalyst found in nature (4).…”

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confidence: 99%

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Oral delivery of RNase P ribozymes by Salmonella inhibits viral infection in mice

Bai¹,

Gong

et al. 2011

Proc. Natl. Acad. Sci. U.S.A.

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Safe, effective, and tissue-specific delivery is a central issue for the therapeutic application of nucleic-acid-based gene interfering agents, such as ribozymes and siRNAs. In this study, we constructed a functional RNase P-based ribozyme (M1GS RNA) that targets the overlapping mRNA region of M80.5 and protease, two murine cytomegalovirus (MCMV) proteins essential for viral replication. In addition, a novel attenuated strain of Salmonella, which exhibited efficient gene transfer activity and little cytotoxicity and pathogenicity in mice, was constructed and used for delivery of anti-MCMV ribozyme. In MCMV-infected macrophages treated with the constructed attenuated Salmonella strain carrying the functional M1GS RNA construct, we observed an 80-85% reduction in the expression of M80.5/protease and a 2,500-fold reduction in viral growth. Oral inoculation of the attenuated Salmonella strain in mice efficiently delivered antiviral M1GS RNA into spleens and livers, leading to substantial expression of the ribozyme without causing significant adverse effects in the animals. Furthermore, the MCMV-infected mice that were treated orally with Salmonella carrying the functional M1GS sequence displayed reduced viral gene expression, decreased viral titers, and improved survival compared to the untreated mice or mice treated with Salmonella containing control ribozyme sequences. Our results provide direct evidence that oral delivery of M1GS RNA by Salmonella-based vectors effectively inhibits viral gene expression and replication in mice. Moreover, this study demonstrates the utility of Salmonellamediated oral delivery of RNase P ribozyme for gene-targeting applications in vivo.gene therapy | herpesvirus | gene delivery | antisense | animal model

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Multiple structural flavors of RNase P in precursor tRNA processing

Sridhara

2024

WIREs RNA

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The precursor transfer RNAs (pre‐tRNAs) require extensive processing to generate mature tRNAs possessing proper fold, structural stability, and functionality required to sustain cellular viability. The road to tRNA maturation follows an ordered process: 5′‐processing, 3′‐processing, modifications at specific sites, if any, and 3′‐CCA addition before aminoacylation and recruitment to the cellular protein synthesis machinery. Ribonuclease P (RNase P) is a universally conserved endonuclease in all domains of life, performing the hydrolysis of pre‐tRNA sequences at the 5′ end by the removal of phosphodiester linkages between nucleotides at position −1 and +1. Except for an archaeal species: Nanoarchaeum equitans where tRNAs are transcribed from leaderless‐position +1, RNase P is indispensable for life and displays fundamental variations in terms of enzyme subunit composition, mechanism of substrate recognition and active site architecture, utilizing in all cases a two metal ion‐mediated conserved catalytic reaction. While the canonical RNA‐based ribonucleoprotein RNase P has been well‐known to occur in bacteria, archaea, and eukaryotes, the occurrence of RNA‐free protein‐only RNase P in eukaryotes and RNA‐free homologs of Aquifex RNase P in prokaryotes has been discovered more recently. This review aims to provide a comprehensive overview of structural diversity displayed by various RNA‐based and RNA‐free RNase P holoenzymes towards harnessing critical RNA–protein and protein–protein interactions in achieving conserved pre‐tRNA processing functionality. Furthermore, alternate roles and functional interchangeability of RNase P are discussed in the context of its employability in several clinical and biotechnological applications.This article is categorized under: RNA Processing > tRNA Processing RNA Evolution and Genomics > RNA and Ribonucleoprotein Evolution RNA Interactions with Proteins and Other Molecules > RNA‐Protein Complexes

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Effective inhibition of human cytomegalovirus gene expression and replication by a ribozyme derived from the catalytic RNA subunit of RNase P from Escherichia coli

Cited by 70 publications

References 35 publications

Characterization of the structure and variability of an internal region of hepatitis C virus RNA for M1 RNA guide sequence ribozyme targeting

Characterization of the structure and variability of an internal region of hepatitis C virus RNA for M1 RNA guide sequence ribozyme targeting

Oral delivery of RNase P ribozymes by Salmonella inhibits viral infection in mice

Multiple structural flavors of RNase P in precursor tRNA processing

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